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Specificity in Glycosylation of Multiple Flagellins by the Modular and Cell

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Specificity in Glycosylation of Multiple Flagellins by the Modular and Cell RESEARCH ARTICLE Specificity in glycosylation of multiple flagellins by the modular and cell cycle regulated glycosyltransferase FlmG Silvia Ardissone†, Nicolas Kint, Patrick H Viollier* Department of Microbiology & Molecular Medicine, Faculty of Medicine / CMU, University of Geneva, Gene`ve, Switzerland Abstract How specificity is programmed into post-translational modification of proteins by glycosylation is poorly understood, especially for O-linked glycosylation systems. Here we reconstitute and dissect the substrate specificity underpinning the cytoplasmic O-glycosylation pathway that modifies all six flagellins, five structural and one regulatory paralog, in Caulobacter crescentus, a monopolarly flagellated alpha-proteobacterium. We characterize the biosynthetic pathway for the sialic acid-like sugar pseudaminic acid and show its requirement for flagellation, flagellin modification and efficient export. The cognate NeuB enzyme that condenses phosphoenolpyruvate with a hexose into pseudaminic acid is functionally interchangeable with other pseudaminic acid synthases. The previously unknown and cell cycle-regulated FlmG protein, a defining member of a new class of cytoplasmic O-glycosyltransferases, is required and sufficient for flagellin modification. The substrate specificity of FlmG is conferred by its N-terminal flagellin- binding domain. FlmG accumulates before the FlaF secretion chaperone, potentially timing flagellin modification, export, and assembly during the cell division cycle. *For correspondence: [email protected] Present address: †Center for Research on Intracellular Introduction Bacteria, Institute of Post-translational protein modification is essential for various facets in cellular biology, ranging from Microbiology, University Hospital Center and University of gene regulation to the organization of cellular structures. In all cases, biological function underlies Lausanne, Bugnon, Switzerland the capacity to specifically identify and modify the correct target protein. Exquisite control mecha- nisms must be in place to ensure modification of the designated target, a feat that is more convo- Competing interest: See luted for proteins that are destined for the cell surface or the exterior, for example, for proteins that page 22 are first modified in the cytosol by dedicated glycosyltransferases (Keys and Aebi, 2017; Funding: See page 22 Nothaft and Szymanski, 2010; Valguarnera et al., 2016). Unraveling the determinants underpin- Received: 27 June 2020 ning the substrate selection is not only important for understanding the fundamentals and diversity Accepted: 24 September 2020 in biological glycosylation systems but also has important translational implications for synthetic biol- Published: 27 October 2020 ogy towards engineering recombinant glycoconjugates as vaccines or glycoproteins in other thera- peutic applications (Nothaft and Szymanski, 2010; Vimr et al., 2004; Cuccui and Wren, 2015; Reviewing editor: Sonja V Albers, University of Freiburg, Ghaderi et al., 2012). Germany In bacteria, extracellular proteinaceous surface structures including pili, flagella, and autotrans- porters as well as toxins are often post-translationally modified by glycosylation (Nothaft and Szy- Copyright Ardissone et al. This manski, 2010; Valguarnera et al., 2016; Vimr et al., 2004; De Maayer and Cowan, 2016; article is distributed under the Miller et al., 2008; Szymanski et al., 2003; Scha¨ffer and Messner, 2017; Goon et al., 2003; terms of the Creative Commons Attribution License, which Schirm et al., 2003; Shen et al., 2006; Sulzenbacher et al., 2018; Lu et al., 2014). Since pili and permits unrestricted use and flagella may be exposed to immune surveillance systems of eukaryotic cells, glycosylation of the redistribution provided that the structural subunits of these appendages, the pilin or flagellin, is often linked to virulence and evasion original author and source are from the host immune system by molecular mimicry (Nothaft and Szymanski, 2010; Scha¨ffer and credited. Messner, 2017; Arora et al., 2005; Logan, 2006). In Salmonella enterica serovar Typhimurium Ardissone et al. eLife 2020;9:e60488. DOI: https://doi.org/10.7554/eLife.60488 1 of 28 Research article Microbiology and Infectious Disease another type of flagellin modification, methylation, was recently shown to promote adhesion to host cells (Horstmann et al., 2020). Flagellin glycosylation may potentially affect flagellar motility in many bacterial lineages since genomic and mass spectrometry data reveal that glycosylation systems are not restricted to pathogens but also occur in non-pathogenic bacteria found in the environment (De Maayer and Cowan, 2016; Schirm et al., 2005). In several polarly flagellated Gram-negative bacteria, flagellin glycosylation is required for assembly of the flagellar filament. In Campylobacter jejuni and Helicobacter pylori, two epsilon-proteobacteria that cause a broad range of human and animal diseases, glycosylation is required for flagellar assembly, motility, and virulence (Schirm et al., 2003; Linton et al., 2000; Guerry et al., 2006; Zebian et al., 2016). H. pylori has a monopolar flagellum, while C. jejuni is bipolarly flagellated (Kostrzynska et al., 1991; Guerry et al., 1991). In Campylobacter species, the exact chemical nature of glycosylation is variable but generally a nine-carbon sugar related to sialic acids such as a pseudaminic acid or legionaminic acid derivative is appended to the flagellin (Thibault et al., 2001; Logan et al., 2002). Many Campylobacter strains possess three dedicated NeuB-like synthases: one for sialic acid (incorporated into the lipo-oligosac- charide), one for legionaminic acid, and one for pseudaminic acid, both used to modify flagellins (Linton et al., 2000; Sundaram et al., 2004; Chou et al., 2005; McNally et al., 2006; McNally et al., 2007; Schoenhofen et al., 2009). By contrast, Helicobacter species seem to use pseudaminic acid only for flagellin glycosylation (McNally et al., 2006; McNally et al., 2007; Schoenhofen et al., 2006). In both C. jejuni and H. pylori, loss of pseudaminic acid biosynthesis results in non-motile strains lacking flagella. The abundance of intracellular flagellin is severely reduced in these mutants and the flagellins showed increased mobility by SDS-PAGE (polyacryl- amide gel electrophoresis), consistent with the loss of glycosylation (Schirm et al., 2003; Linton et al., 2000). Similarly, polar flagellation in the gamma-proteobacteria such as pathogenic Aeromonas spp and the non-pathogenic environmental bacterium Shewanella oneidensis depends on glycosylation of flagellin with pseudaminic acid and another nonulosonic acid derivative, respec- tively (Sun et al., 2013; Schirm et al., 2005; Wilhelms et al., 2012). Interestingly, pseudaminic acid is also a component of surface polysaccharides such as the O-antigen of lipopolysaccharide (LPS) in Aeromonas caviae or the capsular polysaccharide (K antigen) in the symbiotic alpha-proteobacterium Sinorhizobium fredii NGR234 (Forsberg and Reuhs, 1997; Le Que´re´ et al., 2006; Margaret et al., 2012). In A. caviae, the genes required for pseudaminic acid biosynthesis are encoded in the O-anti- gen cluster and their mutation affects both flagellum and LPS O-antigen biosynthesis (Canals et al., 2007; Tabei et al., 2009). The basis for substrate specificity in protein glycosylation systems is poorly understood and ham- pers biotechnological exploitation of these protein modification systems for therapeutic purposes. Flagellin glycosylation occurs at serine or threonine residues by O-linking glycosyltransferases (henceforth OGTs) that modify their substrates to various extent for each flagellin system, ranging from modification at a single site for Burkholderia and Listeria species (Shen et al., 2006; Scott et al., 2011; Hanuszkiewicz et al., 2014) to promiscuous modification at 19 serine or threo- nine residues for the C. jejuni flagellin (Schirm et al., 2005; Thibault et al., 2001). The modification usually occurs at the two surface-exposed central domains of flagellin, ideally positioned to influence the immunogenicity of the filament and the virulence in pathogens (Arora et al., 2005; Verma et al., 2005). Since no consensus sequence determinant in the primary structure of the flagel- lin acceptor (apart from the serine or threonine modification site) has been identified (Thibault et al., 2001), OGTs likely recognize the tertiary structure of the glycosyl acceptor in a highly specific manner. Evidence has been provided that glycosylation precedes secretion of the fla- gellin (Parker et al., 2014) via the flagellar export machinery to the tip of the growing flagellar fila- ment (Chevance and Hughes, 2008). Thus, flagellin identification and subsequent glycosylation by the OGT must occur in the cytoplasm, presumably by soluble proteins. During flagellar assembly in Gram-negative (diderm) bacteria, the basal body harboring the export apparatus is assembled first in the cytoplasmic membrane, followed by envelope-spanning structures along with the external hook structure that serves as universal joint between the flagellar filament and the envelope-span- ning parts (Chevance and Hughes, 2008). The flagellins are assembled last by polymerization on the hook into the flagellar filament (Figure 1A). They are usually the last proteins to be expressed and secreted during assembly, relying on temporal control mechanisms of gene expression promot- ing the orderly assembly of the flagellum. A key feature of polarly
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